JP2015501647A - Active small molecule glue mixture, preparation method and use thereof - Google Patents
Active small molecule glue mixture, preparation method and use thereof Download PDFInfo
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- JP2015501647A JP2015501647A JP2014546275A JP2014546275A JP2015501647A JP 2015501647 A JP2015501647 A JP 2015501647A JP 2014546275 A JP2014546275 A JP 2014546275A JP 2014546275 A JP2014546275 A JP 2014546275A JP 2015501647 A JP2015501647 A JP 2015501647A
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- Prior art keywords
- protease
- small molecule
- glue
- active small
- mixture
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- 239000000203 mixture Substances 0.000 title claims abstract description 61
- 150000003384 small molecules Chemical class 0.000 title claims abstract description 57
- 238000002360 preparation method Methods 0.000 title claims abstract description 10
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- 108091005804 Peptidases Proteins 0.000 claims abstract description 52
- 108090000765 processed proteins & peptides Proteins 0.000 claims abstract description 33
- 239000000463 material Substances 0.000 claims abstract description 21
- ONIBWKKTOPOVIA-BYPYZUCNSA-N L-Proline Chemical compound OC(=O)[C@@H]1CCCN1 ONIBWKKTOPOVIA-BYPYZUCNSA-N 0.000 claims abstract description 20
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- OHDRQQURAXLVGJ-HLVWOLMTSA-N azane;(2e)-3-ethyl-2-[(e)-(3-ethyl-6-sulfo-1,3-benzothiazol-2-ylidene)hydrazinylidene]-1,3-benzothiazole-6-sulfonic acid Chemical compound [NH4+].[NH4+].S/1C2=CC(S([O-])(=O)=O)=CC=C2N(CC)C\1=N/N=C1/SC2=CC(S([O-])(=O)=O)=CC=C2N1CC OHDRQQURAXLVGJ-HLVWOLMTSA-N 0.000 description 5
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- HMUNWXXNJPVALC-UHFFFAOYSA-N 1-[4-[2-(2,3-dihydro-1H-inden-2-ylamino)pyrimidin-5-yl]piperazin-1-yl]-2-(2,4,6,7-tetrahydrotriazolo[4,5-c]pyridin-5-yl)ethanone Chemical compound C1C(CC2=CC=CC=C12)NC1=NC=C(C=N1)N1CCN(CC1)C(CN1CC2=C(CC1)NN=N2)=O HMUNWXXNJPVALC-UHFFFAOYSA-N 0.000 description 1
- VZSRBBMJRBPUNF-UHFFFAOYSA-N 2-(2,3-dihydro-1H-inden-2-ylamino)-N-[3-oxo-3-(2,4,6,7-tetrahydrotriazolo[4,5-c]pyridin-5-yl)propyl]pyrimidine-5-carboxamide Chemical compound C1C(CC2=CC=CC=C12)NC1=NC=C(C=N1)C(=O)NCCC(N1CC2=C(CC1)NN=N2)=O VZSRBBMJRBPUNF-UHFFFAOYSA-N 0.000 description 1
- SXAMGRAIZSSWIH-UHFFFAOYSA-N 2-[3-[2-(2,3-dihydro-1H-inden-2-ylamino)pyrimidin-5-yl]-1,2,4-oxadiazol-5-yl]-1-(2,4,6,7-tetrahydrotriazolo[4,5-c]pyridin-5-yl)ethanone Chemical compound C1C(CC2=CC=CC=C12)NC1=NC=C(C=N1)C1=NOC(=N1)CC(=O)N1CC2=C(CC1)NN=N2 SXAMGRAIZSSWIH-UHFFFAOYSA-N 0.000 description 1
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- YJLUBHOZZTYQIP-UHFFFAOYSA-N 2-[5-[2-(2,3-dihydro-1H-inden-2-ylamino)pyrimidin-5-yl]-1,3,4-oxadiazol-2-yl]-1-(2,4,6,7-tetrahydrotriazolo[4,5-c]pyridin-5-yl)ethanone Chemical compound C1C(CC2=CC=CC=C12)NC1=NC=C(C=N1)C1=NN=C(O1)CC(=O)N1CC2=C(CC1)NN=N2 YJLUBHOZZTYQIP-UHFFFAOYSA-N 0.000 description 1
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- USHAGKDGDHPEEY-UHFFFAOYSA-L potassium persulfate Chemical compound [K+].[K+].[O-]S(=O)(=O)OOS([O-])(=O)=O USHAGKDGDHPEEY-UHFFFAOYSA-L 0.000 description 1
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Images
Classifications
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K38/00—Medicinal preparations containing peptides
- A61K38/01—Hydrolysed proteins; Derivatives thereof
- A61K38/012—Hydrolysed proteins; Derivatives thereof from animals
- A61K38/014—Hydrolysed proteins; Derivatives thereof from animals from connective tissue peptides, e.g. gelatin, collagen
-
- A—HUMAN NECESSITIES
- A23—FOODS OR FOODSTUFFS; TREATMENT THEREOF, NOT COVERED BY OTHER CLASSES
- A23L—FOODS, FOODSTUFFS, OR NON-ALCOHOLIC BEVERAGES, NOT COVERED BY SUBCLASSES A21D OR A23B-A23J; THEIR PREPARATION OR TREATMENT, e.g. COOKING, MODIFICATION OF NUTRITIVE QUALITIES, PHYSICAL TREATMENT; PRESERVATION OF FOODS OR FOODSTUFFS, IN GENERAL
- A23L33/00—Modifying nutritive qualities of foods; Dietetic products; Preparation or treatment thereof
- A23L33/10—Modifying nutritive qualities of foods; Dietetic products; Preparation or treatment thereof using additives
- A23L33/17—Amino acids, peptides or proteins
- A23L33/18—Peptides; Protein hydrolysates
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K35/00—Medicinal preparations containing materials or reaction products thereof with undetermined constitution
- A61K35/12—Materials from mammals; Compositions comprising non-specified tissues or cells; Compositions comprising non-embryonic stem cells; Genetically modified cells
- A61K35/36—Skin; Hair; Nails; Sebaceous glands; Cerumen; Epidermis; Epithelial cells; Keratinocytes; Langerhans cells; Ectodermal cells
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K47/00—Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient
- A61K47/30—Macromolecular organic or inorganic compounds, e.g. inorganic polyphosphates
- A61K47/42—Proteins; Polypeptides; Degradation products thereof; Derivatives thereof, e.g. albumin, gelatin or zein
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P39/00—General protective or antinoxious agents
- A61P39/06—Free radical scavengers or antioxidants
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P7/00—Drugs for disorders of the blood or the extracellular fluid
-
- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K14/00—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
- C07K14/435—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
- C07K14/78—Connective tissue peptides, e.g. collagen, elastin, laminin, fibronectin, vitronectin or cold insoluble globulin [CIG]
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- Health & Medical Sciences (AREA)
- Life Sciences & Earth Sciences (AREA)
- Chemical & Material Sciences (AREA)
- Medicinal Chemistry (AREA)
- Engineering & Computer Science (AREA)
- General Health & Medical Sciences (AREA)
- Public Health (AREA)
- Veterinary Medicine (AREA)
- Animal Behavior & Ethology (AREA)
- Pharmacology & Pharmacy (AREA)
- Proteomics, Peptides & Aminoacids (AREA)
- Epidemiology (AREA)
- Zoology (AREA)
- Organic Chemistry (AREA)
- Immunology (AREA)
- Biomedical Technology (AREA)
- Cell Biology (AREA)
- Molecular Biology (AREA)
- Bioinformatics & Cheminformatics (AREA)
- Biochemistry (AREA)
- Toxicology (AREA)
- Biotechnology (AREA)
- Virology (AREA)
- Developmental Biology & Embryology (AREA)
- Dermatology (AREA)
- Food Science & Technology (AREA)
- Polymers & Plastics (AREA)
- Chemical Kinetics & Catalysis (AREA)
- Inorganic Chemistry (AREA)
- General Chemical & Material Sciences (AREA)
- Mycology (AREA)
- Nutrition Science (AREA)
- Nuclear Medicine, Radiotherapy & Molecular Imaging (AREA)
- Gastroenterology & Hepatology (AREA)
- Biophysics (AREA)
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- Diabetes (AREA)
- Hematology (AREA)
- Coloring Foods And Improving Nutritive Qualities (AREA)
- Preparation Of Compounds By Using Micro-Organisms (AREA)
Abstract
活性小分子阿膠混合物、並びに、その調製方法及び用途。前記活性小分子阿膠混合物は、プロリンプロテアーゼを含む複合プロテアーゼを用いて、補助材が加えられていない阿膠液の酵素加水分解を行うことによって調製する。前記活性小分子阿膠混合物は、重量平均分子量が580Da〜1300Daの範囲であり、ペプチド部分が200Da〜3000Daに分布しており、冷水への溶解速度が速く、遊離アミノ酸の含有量が少なく、前記活性小分子阿膠混合物は、阿膠の小分子ペプチド食品及び保険食品の製造に用いてよい。【選択図】図1Active small molecule glue mixture, and its preparation and use. The active small molecule glue mixture is prepared by enzymatic hydrolysis of glue liquor to which no auxiliary material has been added, using a complex protease containing proline protease. The active small molecule glue mixture has a weight average molecular weight in the range of 580 Da to 1300 Da, a peptide portion distributed in 200 Da to 3000 Da, a high dissolution rate in cold water, a low free amino acid content, and the activity The small molecule glue mixture may be used in the production of small molecule peptide foods and insurance foods for glue. [Selection] Figure 1
Description
本発明は、活性小分子混合物、並びに、その調製方法及び用途に関し、具体的には、阿膠液の酵素加水分解により得られる活性小分子ペプチド混合物、並びに、その適用方法及び用途に関する。本発明は、食品バイオテクノロジーの分野に属する。 The present invention relates to an active small molecule mixture, and a preparation method and use thereof. Specifically, the present invention relates to an active small molecule peptide mixture obtained by enzymatic hydrolysis of glue liquid, and an application method and use thereof. The present invention belongs to the field of food biotechnology.
阿膠は、血液を補い、気を養うのに有効な薬物である。阿膠は、後漢の時代に早くも、高名な薬物書「神農本草経」に「上品」として記載されているとともに、「長期間服用すると、気を補い、身体を軽く感じるようになる」と書かれている。阿膠の特徴は「甘」、「平」であり、その主な機能は、血液を補うとともに、陰を養って、乾燥状態を改善し、止血することである。阿膠は、血液不足による皮膚の黄化、めまい、動悸、筋委縮及び脱力、情緒的過敏、不眠、虚風内動、肺の乾燥による咳、労咳、喀血、吐血及び血尿、血便、切迫流産等を治療するのに用いる。2010年版中国薬典によれば、阿膠は、ウマ科のロバの乾皮又は未加工の皮膚を煮てから、その煎出物を濃縮することによって作られる固体ゼラチンである。しかしながら、コラーゲンタンパク質の分子量は非常に大きく(数万〜数十万)、脾臓及び胃の弱い患者は吸収できず、その結果、阿膠の機能が充分に発揮されない。同時に、近年、ロバの飼育頭数が減っており、これにより、必然的にロバの皮膚の供給量が不足するとともに、阿膠の価格が上昇している。ロバの皮膚材の深刻化する供給不足のため、市場の需要を満たすことができないが、阿膠液の酵素加水分解によって得られる小分子阿膠は、阿膠の生物学的利用能を大幅に高めることができるので、供給と需要のギャップを解消するための良好な手段となり得る。 Ag is an effective drug that supplements the blood and nurtures it. As early as in the later Han Dynasty, Akagi was described as “elegant” in the prestigious drug book “Shinnohonhon Sukei”, and “If you take it for a long time, you will feel better and feel lighter”. has been written. The characteristics of Aji are “sweet” and “flat”, and its main function is to supplement the blood, nourish the shade, improve the dry state, and stop bleeding. Ag is skin yellowing due to lack of blood, dizziness, palpitation, muscle atrophy and weakness, emotional hypersensitivity, insomnia, internal movement of the wind, cough due to dryness of the lungs, labor cough, hemoptysis, vomiting and hematuria, bloody stool, imminent abortion, etc. Used to treat. According to the 2010 Chinese Pharmacy, Aji is a solid gelatin made by boiling dry or raw skin of equine donkeys and then concentrating the decoction. However, the molecular weight of collagen protein is very large (tens of thousands to hundreds of thousands), and patients with weak spleen and stomach cannot be absorbed, and as a result, the function of glue is not fully exhibited. At the same time, the number of donkeys has been bred in recent years, which inevitably leads to a shortage of donkey skin supply and increases in the price of glue. Due to the growing supply of donkey skin material, the market demand cannot be met, but small molecule glue obtained by enzymatic hydrolysis of glue fluid can greatly increase the bioavailability of glue. It can be a good way to close the gap between supply and demand.
近年、阿膠の酵素分解に関する研究はいくらか進展しており、(1)中国特許出願公開第1237421A号「酵素分解による液体阿膠の調製方法」、(2)中国特許出願公開第1807653A号「活性阿膠コラーゲンペプチド生成物」、(3)中国特許出願公開第101269090A号「低分子量を有する阿膠加水分解物の調製方法」を含め、多くの特許が公開されている。これらの3つの発明はいずれも、阿膠のプロテアーゼ消化によるコラーゲンペプチドの作製を報告している。既存の技術に基づき、本発明は、阿膠における特徴的に高いプロリン及びヒドロキシプロリン含有量を利用して、初めて、プロリンプロテアーゼを用いて阿膠を酵素消化することを提案し、その結果、過去の特許で報告されたものよりも、加水分解効果が有意に高くなる。上述の3つの特許では、大半の生成物の分子量は、5000Da未満、更には10000Da未満の範囲に分布していた。加えて、上記のいずれの特許でも、分子量分布と遊離アミノ酸含有量の正確な測定結果は報告されていないが、本発明では、ペプチド分子量は200〜3000Daの範囲、主に200〜1000Daの範囲に分布している。中国特許出願公開第1237421A号及び中国特許出願公開第1807653A号では、いずれも、消化原料として加えた補助材とともに、阿膠の塊を用いていたが、本発明では、プロセスを簡素化し、コストを抑え、良好な溶解性と高い生物学的利用能を有する生成物を得るために、酵素分解の原料として阿膠液を用いており、DPPHラジカル及びABTSラジカルの消去率は100%に近い。 In recent years, some researches on the enzymatic degradation of glue have made some progress: (1) Chinese Patent Application No. 1237421A “Method of preparing liquid glue by enzymatic degradation”, (2) Chinese Patent Application Publication No. 1807653A “Active collagen collagen Numerous patents have been published, including "Peptide Products", (3) Chinese Patent Application No. 1012669090A "Method for preparing low-molecular weight glue hydrolyzate". All three inventions report the production of collagen peptides by protease digestion of glue. Based on the existing technology, the present invention proposes to enzymatically digest Ag with proline protease for the first time, utilizing the characteristically high proline and hydroxyproline content in Ag, and as a result, the past patents The hydrolysis effect is significantly higher than that reported in. In the three patents mentioned above, the molecular weight of most products was distributed in the range of less than 5000 Da and even less than 10,000 Da. In addition, in any of the above patents, accurate measurement results of molecular weight distribution and free amino acid content are not reported, but in the present invention, the peptide molecular weight is in the range of 200 to 3000 Da, mainly in the range of 200 to 1000 Da. Distributed. In both Chinese Patent Application Publication No. 1237421A and Chinese Patent Application Publication No. 1807653A, the lump of glue is used together with the auxiliary material added as a digestion raw material, but in the present invention, the process is simplified and the cost is reduced. In order to obtain a product having good solubility and high bioavailability, glue solution is used as a raw material for enzymatic degradation, and the DPPH radical and ABTS radical elimination rates are close to 100%.
文献(Adibi A S.America Nutrition,1984,25:1114−1122、DBA Silk Gut,1974,15:494−501)内の多くの報告では、分子量が200〜1000Daの範囲であるペプチドは、他のサイズのペプチド及び遊離アミノ酸よりも、吸収性及び効能が優れていることが示されている。本発明は、生成物中の遊離アミノ酸含有量と、生成物の分子量分布を正確に割り出すために、原料としての補助材なしに阿膠液を用いることを提案し、生成物に含まれる小ペプチドは大体、200〜1000Daの範囲に分布するので、吸収性と効能が高い。 In many reports in the literature (Adivi AS S. America Nutrition, 1984, 25: 1114-1122, DBA Silk Gut, 1974, 15: 494-501), peptides with molecular weights in the range of 200-1000 Da are Absorption and efficacy have been shown to be superior to size peptides and free amino acids. The present invention proposes the use of glue liquid without auxiliary materials as raw materials in order to accurately determine the content of free amino acids in the product and the molecular weight distribution of the product, and the small peptide contained in the product is Since it is generally distributed in the range of 200 to 1000 Da, the absorbency and efficacy are high.
既存の技法における問題を解決するために、本発明の目的の1つは、活性小分子阿膠混合物を提供することである。 In order to solve the problems in existing techniques, one of the objects of the present invention is to provide active small molecule glue mixtures.
本発明の第2の目的は、活性小分子阿膠混合物の作製方法を提供することである。 The second object of the present invention is to provide a method for preparing active small molecule glue mixtures.
本発明の第3の目的は、小分子ペプチド食品及び健康食品の製造に前記活性小分子阿膠混合物を適用することを提供することである。 The third object of the present invention is to provide application of the active small molecule glue mixture to the production of small molecule peptide foods and health foods.
上記の目的を達成するために、本発明では、下記の技術的手段を採用する。 In order to achieve the above object, the present invention employs the following technical means.
本発明で提案する活性小分子阿膠混合物であって、生成物の重量平均分子量が580〜1300Daであり、ペプチドが、200〜3000Da、主に200〜1000Daに分布する活性小分子阿膠混合物。 An active small molecule glue mixture proposed in the present invention, wherein the product has a weight average molecular weight of 580 to 1300 Da, and peptides are distributed in 200 to 3000 Da, mainly 200 to 1000 Da.
本発明では、複合プロテアーゼを用いて阿膠液の酵素加水分解を行うことによって、活性小分子阿膠混合物を調製する。前記複合プロテアーゼは、パパイン及びプロリンプロテアーゼを含み、前記複合プロテイナーゼは更に、ブロメラインプロテアーゼ、中性プロテアーゼ、ペプシン、及びフレーバーザイムからなる群から選択したプロテアーゼを1つ、又は複数、又は全て含むのが好ましい。 In the present invention, an active small molecule glue mixture is prepared by enzymatic hydrolysis of glue liquid using a complex protease. Preferably, the complex protease includes papain and proline protease, and the complex proteinase further includes one, a plurality, or all of a protease selected from the group consisting of bromelain protease, neutral protease, pepsin, and flavorzyme. .
本発明では、前記活性小分子阿膠混合物を処理して粉末又は液体製剤にすることができる。 In the present invention, the active small molecule glue mixture can be processed into a powder or liquid preparation.
本発明で提案する活性小分子阿膠混合物の特徴は、(1)処理して経口投与用の粉末又は液体製剤にできること、(2)溶解性が良好で、冷水への溶解速度も速いこと、(3)遊離アミノ酸の含有量が少なく(わずか4%)、分子量が200〜1000Daの範囲である小ペプチドが全体の81%を占め、1000〜3000Daのペプチドが14%を占め(図1参照)、重量平均分子量が765Daであること、(4)生物学的利用能については、小分子阿膠の生物学的利用能が、通常の阿膠の3.5倍であり、生物消化した阿膠の2.2倍であること(図2参照)、(5)抗酸化効果の面では、小分子阿膠は、DPPH及びABTSを含むラジカルを除去する優れた効能を有し、10mg/mlの濃度で、消去率を100%近くにできること(図3及び4参照)である。 The characteristics of the active small molecule glue mixture proposed in the present invention are as follows: (1) it can be processed into a powder or liquid preparation for oral administration; (2) it has good solubility and a high dissolution rate in cold water; 3) Small peptides with low free amino acid content (only 4%) and molecular weights in the range of 200-1000 Da accounted for 81% of the total, 1000-3000 Da peptides accounted for 14% (see FIG. 1), (4) Regarding bioavailability, the bioavailability of small molecule glue is 3.5 times that of normal glue, and 2.2 of biodigested glue. (5) In terms of antioxidant effect, small molecule glue has an excellent effect of removing radicals including DPPH and ABTS, and has an erasure rate of 10 mg / ml. Can be close to 100% A (see FIGS. 3 and 4).
本発明は、活性小分子阿膠混合物を作製する方法であって、
(1)補助材を含まない阿膠液を室温で30〜55℃まで冷まし、pHを5〜8に調節し、この液に複合プロテアーゼを加えて、加水分解反応を0.5〜2時間行うことによって、阿膠液の加水分解物を得る工程と、
(2)工程(1)で得た阿膠液の加水分解物を10〜30分間煮て、上記の酵素を不活性化することによって、不活性化煎出物を得る工程と、
(3)この不活性化煎出物を遠心分離して不純物を除去することによって、活性小分子阿膠混合物の液体製剤を得る工程と、
を含む方法も提供する。
The present invention is a method of making an active small molecule glue mixture comprising:
(1) Cool the glue solution not containing auxiliary materials to 30-55 ° C. at room temperature, adjust the pH to 5-8, add complex protease to this solution, and perform the hydrolysis reaction for 0.5-2 hours. To obtain a hydrolyzate of agar liquid,
(2) A step of obtaining an inactivated decoction by incubating the hydrolyzate of the glue liquid obtained in step (1) for 10 to 30 minutes to inactivate the enzyme,
(3) obtaining a liquid formulation of active small molecule glue mixture by centrifuging the inactivated decoction to remove impurities;
A method is also provided.
本発明で提案する前記活性小分子阿膠混合物を調製するための方法は、前記液体製剤を噴霧乾燥して、活性小分子阿膠混合物の粉末製剤を作製する工程を更に含んでもよい。 The method for preparing the active small molecule glue mixture proposed in the present invention may further include the step of spray-drying the liquid preparation to produce a powder formulation of the active small molecule glue mixture.
本発明で提案する方法では、前記補助材は、黄酒、氷砂糖、及び大豆油を含み、前記補助材を含まない阿膠液は、黄酒、氷砂糖、又は大豆油が無添加の阿膠液である。 In the method proposed in the present invention, the auxiliary material includes yellow liquor, rock sugar, and soybean oil, and the gelatin liquid not including the auxiliary material is a glue liquid that does not contain yellow wine, rock sugar, or soybean oil.
本発明の実施形態では、工程(1)における阿膠液の濃度は10%〜50%(w/w)である。 In the embodiment of the present invention, the concentration of the glue liquid in the step (1) is 10% to 50% (w / w).
本発明の実施形態では、前記複合プロテアーゼは、パパイン及びプロリンプロテアーゼを含み、前記複合プロテイナーゼは更に、ブロメラインプロテアーゼ、中性プロテアーゼ、ペプシン、及びフレーバーザイムからなる群から選択したプロテアーゼを1つ、又は複数、又は全て含むのが好ましい。 In an embodiment of the present invention, the complex protease includes papain and proline protease, and the complex proteinase further includes one or more proteases selected from the group consisting of bromelain protease, neutral protease, pepsin, and flavorzyme. Or all.
工程(1)で加える複合プロテアーゼの量が阿膠液の5重量%〜3重量%(w/w)である本発明の実施形態では、複合プロテアーゼの添加順については、上記の酵素を順に一定の間隔で加えるか、又は、加水分解反応の初期段階に、上記の酵素を同時に加えるかである。 In the embodiment of the present invention in which the amount of the complex protease added in the step (1) is 5% by weight to 3% by weight (w / w) of the glue solution, the order of addition of the complex protease is constant for the enzymes described above. Either at intervals or at the initial stage of the hydrolysis reaction, the above enzymes are added simultaneously.
本発明の特定の実施形態では、重量によれば、複合プロテアーゼの各々の添加比は、パパイン:プロリンプロテアーゼ=2:1、又はパパイン:プロリンプロテアーゼ:ブロメライン、中性プロテアーゼ、ペプシン、若しくはフレーバーザイムのいずれか1つ=5:2:1である。その他の比については詳述しない。当業者は、いかなる創造的作業もせずに、適用時の実際の状況に基づき、多種多様な選択をすることができる。 In certain embodiments of the invention, by weight, each addition ratio of complex proteases is papain: proline protease = 2: 1, or papain: proline protease: bromelain, neutral protease, pepsin, or flavorzyme. Any one = 5: 2: 1. Other ratios are not described in detail. A person skilled in the art can make a wide variety of choices based on the actual situation at the time of application without any creative work.
本発明は更に、活性小分子阿膠混合物を小分子ペプチド食品及び健康食品の調製に適用することを提供する。小分子活性ペプチド混合物により、吸収性が向上し、非常に良好な溶解性と非常に良好な抗酸化効果を示すので、粉末又は液体製剤の食品、並びに、抗酸化機能及び老化遅延機能を有する健康食品の開発に有用である。 The present invention further provides the application of active small molecule glue mixtures to the preparation of small molecule peptide foods and health foods. Small molecule active peptide mixture improves absorption, shows very good solubility and very good anti-oxidant effect, so foods in powder or liquid formulation and health with anti-oxidation and aging delay Useful for food development.
既存の技法と比べた場合の本発明の利点は以下のとおりである。 The advantages of the present invention over existing techniques are as follows.
1:提案する方法は、いずれの補助材も原料として含まない阿膠液を用いることによって、プロセスの簡易化、省エネルギー、コスト削減、高効率の加水分解、並びに、噴霧乾燥生成物の構造及び特性の安定性の確保をもたらす。 1: The proposed method uses a glue liquid that does not contain any auxiliary material as a raw material, thereby simplifying the process, saving energy, reducing costs, highly efficient hydrolysis, and the structure and properties of the spray-dried product. It will ensure stability.
2:提案する方法は、遠心分離によって生成物中の脂肪及び不純物を取り除き、生成物の溶解性が高くなるように、かつ、生成物が、関連する食品及び健康食品の開発の助けとなるようにする。 2: The proposed method removes fats and impurities in the product by centrifugation, so that the product is highly soluble, and the product helps the development of related foods and health foods To.
3:提案する方法では、噴霧乾燥を用いて粉末原料を得て、低い保管コストと、カプセル剤及び顆粒製品の開発しやすさを確保する。 3: In the proposed method, the powder raw material is obtained using spray drying to ensure low storage costs and ease of development of capsules and granule products.
4:提案する方法では、生成物の試験技法を進歩させ、遊離アミノ酸の含有量とペプチドの分布を正確に割り出せるようにする。 4: The proposed method advances product testing techniques so that the free amino acid content and peptide distribution can be accurately determined.
5:提案する方法では、酵素分解技術が進展し、生成物中のペプチドの分子量は主に200〜1000Daに分布しており、この分子量範囲は、公開されているプロセスによって得られるものよりも低く、これにより、更に高い吸収性と機能的効果が確保される。 5: In the proposed method, the enzymatic degradation technology has progressed, the molecular weight of peptides in the product is mainly distributed in the range of 200-1000 Da, this molecular weight range is lower than that obtained by published processes This ensures higher absorbency and functional effects.
6:本発明で提案する作製技術は進展しているとともに、実用的であり、阿膠から高収率の小分子混合物が確保される。例えば、原料として40%阿膠液を1L用いて、酵素分解とその後のプロセスの後に得られた粉末生成物は約360gで、収率は90%であった。 6: The production technique proposed in the present invention is advanced and practical, and a high-molecular-weight mixture with high yield is secured from the glue. For example, using 1 L of 40% glue solution as a raw material, the powder product obtained after the enzymatic decomposition and the subsequent process was about 360 g, and the yield was 90%.
7:得られた物質の生物学的利用能と抗酸化効果を予備的に割り出したところ、非常に良好な結果を示した。 7: Preliminary determination of the bioavailability and antioxidant effect of the obtained substance showed very good results.
以下では、本発明を実施形態によって更に説明する。本発明の長所及び特徴は、この説明によって明らかになる。これらの実施形態は実例に過ぎず、本発明の保護範囲を制限するものでは決してないと理解されたい。当業者であれば、本発明の趣旨及び範囲から逸脱せずに、本発明の細部及び形状を修正又は置換できることが分かるであろうし、そのような修正形態及び置換形態はいずれも、本発明の保護範囲内である。 In the following, the present invention will be further explained by embodiments. The advantages and features of the invention will become apparent from this description. It should be understood that these embodiments are illustrative only and do not in any way limit the scope of protection of the present invention. Those skilled in the art will recognize that the details and shape of the invention can be modified or replaced without departing from the spirit and scope of the invention, and all such modifications and substitutions are Within protection range.
本発明の実施形態に関連する実験材料の供給源は以下のとおりである。 The sources of experimental material relevant to the embodiments of the present invention are as follows.
1:黄酒、氷砂糖、及び大豆油を含まない阿膠液は、Shandong Dong−E Donkey−hide gelatin Co.,Ltd.から購入した。 1: Astringent fluid without yellow liquor, rock sugar, and soybean oil was obtained from Shandong Dong-E Donkey-hide gelatin Co. , Ltd., Ltd. Purchased from.
2:各種酵素
フレーバーザイム、中性プロテアーゼ、及びブロメラインは、Pangbo Bioengineering Co.,Ltd.,Nanning,Chinaから購入し、パパイン及びペプシンは、Keyuan Industrial Co.,Ltd.から購入し、プロリンプロテアーゼはShanghai Yuanda Business Ltd.から購入した。
2: Various enzymes Flavorzyme, neutral protease, and bromelain were obtained from Pangbo Bioengineering Co. , Ltd., Ltd. Papain and pepsin were purchased from Keyuan Industrial Co., Ltd., Nanning, China. , Ltd., Ltd. Proline protease was purchased from Shanhai Yuanda Business Ltd. Purchased from.
3:ABTSラジカル及びDPPHラジカルは、Sigma Aldrich Co.,Ltd.から購入した。 3: ABTS radical and DPPH radical are available from Sigma Aldrich Co. , Ltd., Ltd. Purchased from.
実施例1
補助材を加えていない1Lの阿膠液(40%(w/w))を室温で35℃まで冷まし、そのpHを6.5に調節した。この液に、5%(w/w)の複合プロテアーゼ(パパイン:プロリンプロテアーゼ=2:1(w/w))を加え、加水分解反応を2時間行い、この液を煮るために加熱し、20分間煮続けて上記の酵素を不活性化してから、遠心分離して不溶性不純物と脂肪を除去して、活性小分子阿膠混合物の液体調製物を得た。この生成物の分子量を割り出したところ、ペプチドの大半は200〜3000Daの範囲であり、全体の83%を占めた。
Example 1
1 L of glue liquid (40% (w / w)) without added auxiliary material was cooled to 35 ° C. at room temperature, and its pH was adjusted to 6.5. To this solution, 5% (w / w) complex protease (papain: proline protease = 2: 1 (w / w)) was added, a hydrolysis reaction was carried out for 2 hours, and this solution was heated to boil, Boiled for a minute to inactivate the above enzyme and then centrifuged to remove insoluble impurities and fat to obtain a liquid preparation of active small molecule glue mixture. When the molecular weight of this product was determined, most of the peptides ranged from 200 to 3000 Da, accounting for 83% of the total.
実施例2
補助材を加えていない1Lの阿膠液(40%(w/w))を室温で35℃まで冷まし、そのpHを6.5に調節した。この液に、5%(w/w)の複合プロテアーゼ(パパイン:プロリンプロテアーゼ=2:1(w/w))を加え、加水分解反応を2時間行い、この液を20分間煮続けて上記の酵素を不活性化してから、遠心分離して不溶性不純物と脂肪を除去し、最後にこの液体を噴霧乾燥して、360gの粉末活性小分子阿膠混合物を得た。この生成物の分子量を割り出したところ、ペプチドの大半は200〜3000Daの範囲であり、全体の83%を占めた。
Example 2
1 L of glue liquid (40% (w / w)) without added auxiliary material was cooled to 35 ° C. at room temperature, and its pH was adjusted to 6.5. To this solution, 5% (w / w) complex protease (papain: proline protease = 2: 1 (w / w)) was added, the hydrolysis reaction was performed for 2 hours, and this solution was boiled for 20 minutes, The enzyme was inactivated and then centrifuged to remove insoluble impurities and fat, and finally the liquid was spray dried to give 360 g of powdered active small molecule glue mixture. When the molecular weight of this product was determined, most of the peptides ranged from 200 to 3000 Da, accounting for 83% of the total.
実施例3
補助材を加えていない1Lの阿膠液(40%(w/w))を室温で40℃まで冷まし、そのpHを5.5に調節した。この液に1%(w/w)の複合プロテアーゼ(パパイン:プロリンプロテアーゼ:ペプシン=5:2:1(w/w))を加えて、加水分解反応を2時間行い、この液を20分間煮続けて上記の酵素を不活性化してから、遠心分離して不溶性不純物と脂肪を除去し、最後にこの液体を噴霧乾燥して、360gの粉末活性小分子阿膠混合物を得た。この生成物の分子量を割り出したところ、ペプチドの大半は200〜3000Daの範囲であり、全体の86%を占めた。
Example 3
1 L of glue liquid (40% (w / w)) without added auxiliary material was cooled to 40 ° C. at room temperature, and its pH was adjusted to 5.5. 1% (w / w) complex protease (papain: proline protease: pepsin = 5: 2: 1 (w / w)) was added to this solution, and the hydrolysis reaction was carried out for 2 hours, and this solution was boiled for 20 minutes. Subsequently, the enzyme was inactivated, and then centrifuged to remove insoluble impurities and fat. Finally, the liquid was spray-dried to obtain 360 g of powdered active small molecule glue mixture. When the molecular weight of this product was determined, the majority of peptides ranged from 200 to 3000 Da, accounting for 86% of the total.
実施例4
補助材を加えていない1Lの阿膠液(10%(w/w))を室温で35℃まで冷まし、そのpHを6に調節した。この液に2%(w/w)の複合プロテアーゼ(パパイン:プロリンプロテアーゼ:中性プロテアーゼ:ペプシン:フレーバーザイム=6:3:1:1:1(w/w))を加え、加水分解反応を2時間行い、この液を20分間煮続けて上記の酵素を不活性化してから、遠心分離して不溶性不純物と脂肪を除去し、最後にその液体を噴霧乾燥して、360gの粉末活性小分子阿膠混合物を得た。この生成物の分子量を割り出したところ、ペプチドの大半は200〜3000Daの範囲であり、全体の75%を占めた。
Example 4
1 L of glue liquid (10% (w / w)) without added auxiliary material was cooled to 35 ° C. at room temperature, and its pH was adjusted to 6. 2% (w / w) of complex protease (papain: proline protease: neutral protease: pepsin: flavorzyme = 6: 3: 1: 1: 1 (w / w)) was added to this solution to conduct hydrolysis reaction. Incubate for 2 hours and boil this solution for 20 minutes to inactivate the enzymes, then centrifuge to remove insoluble impurities and fat, and finally spray dry the liquid to give 360 g of powdered small active molecule An adhesive mixture was obtained. When the molecular weight of this product was determined, most of the peptides ranged from 200 to 3000 Da, accounting for 75% of the total.
実施例5
補助材を加えていない1Lの阿膠液(40%(w/w))を室温で50℃まで冷まし、そのpHを6.5に調節した。この液に3%(w/w)の複合プロテアーゼ(パパイン:プロリンプロテアーゼ:ペプシン:中性プロテアーゼ:フレーバーザイム=6:2:2:1:1(w/w))を加え、加水分解反応を2時間行い、この液を20分間煮続けて上記の酵素を不活性化してから、遠心分離して不溶性不純物と脂肪を除去し、最後にその液体を噴霧乾燥して、360gの粉末活性小分子阿膠混合物を得た。この生成物の分子量を割り出したところ、ペプチドの大半は200〜3000Daの範囲であり、全体の95%を占めた。
Example 5
1 L of glue liquid (40% (w / w)) without added auxiliary material was cooled to 50 ° C. at room temperature, and its pH was adjusted to 6.5. 3% (w / w) complex protease (papain: proline protease: pepsin: neutral protease: flavorzyme = 6: 2: 2: 1: 1 (w / w)) was added to this solution, and the hydrolysis reaction was performed. Incubate for 2 hours and boil this solution for 20 minutes to inactivate the enzymes, then centrifuge to remove insoluble impurities and fat, and finally spray dry the liquid to give 360 g of powdered small active molecule An adhesive mixture was obtained. When the molecular weight of this product was determined, most of the peptides ranged from 200 to 3000 Da, accounting for 95% of the total.
実施例6
補助材を加えていない1Lの阿膠液(40%(w/w))を室温で40℃まで冷まし、そのpHを6.5に調節した。この液に3%(w/w)の複合プロテアーゼ(パパイン:プロリンプロテアーゼ:ペプシン:中性プロテアーゼ:フレーバーザイム=6:2:2:1:1(w/w))を加え、加水分解反応を0.5時間行い、この液を煮るために加熱し、20分間煮続けて上記の酵素を不活性化してから、遠心分離して不溶性不純物と脂肪を除去し、最後にこの液体を噴霧乾燥して、360gの粉末活性小分子阿膠混合物を得た。この生成物の分子量を割り出したところ、ペプチドの大半は200〜3000Daであり、全体の83%を占めた。
Example 6
1 L of glue liquid (40% (w / w)) without added auxiliary material was cooled to 40 ° C. at room temperature, and its pH was adjusted to 6.5. 3% (w / w) complex protease (papain: proline protease: pepsin: neutral protease: flavorzyme = 6: 2: 2: 1: 1 (w / w)) was added to this solution, and the hydrolysis reaction was performed. Incubate for 0.5 hour, heat to boil, continue to boil for 20 minutes to inactivate the enzyme, centrifuge to remove insoluble impurities and fat, and finally spray dry the liquid. 360 g of powdered active small molecule glue mixture was obtained. When the molecular weight of this product was determined, most of the peptides were 200-3000 Da, accounting for 83% of the total.
実施例7
補助材を加えていない1Lの阿膠液(40%(w/w))を室温で40℃まで冷まし、そのpHを6.5に調節した。この液に5%(w/w)の複合プロテアーゼ(パパイン:プロリンプロテアーゼ:ペプシン:中性プロテアーゼ:フレーバーザイム=6:2:2:1:1(w/w))を加え、加水分解反応を2時間行い、この液を煮るために加熱し、20分間煮続けて上記の酵素を不活性化してから、遠心分離して不溶性不純物と脂肪を除去し、最後に液体を噴霧乾燥して、360gの粉末活性小分子阿膠混合物を得た。この生成物の分子量を割り出したところ、ペプチドの大半は200〜3000Daであり、全体の71%を占めた。
Example 7
1 L of glue liquid (40% (w / w)) without added auxiliary material was cooled to 40 ° C. at room temperature, and its pH was adjusted to 6.5. 5% (w / w) complex protease (papain: proline protease: pepsin: neutral protease: flavorzyme = 6: 2: 2: 1: 1 (w / w)) was added to this solution, and the hydrolysis reaction was performed. Heated to boil this liquid for 2 hours, boiled for 20 minutes to inactivate the above enzymes, then centrifuged to remove insoluble impurities and fat, and finally the liquid was spray dried to 360 g A powdery active small molecule glue mixture was obtained. When the molecular weight of this product was determined, most of the peptides were 200-3000 Da, accounting for 71% of the total.
実施例8
補助材を加えていない1Lの阿膠液(40%(w/w))を室温で40℃まで冷まし、そのpHを6.5に調節した。この液に1.5%(w/w)の複合プロテアーゼ(パパイン:プロリンプロテアーゼ=2:1(w/w))を加え、加水分解反応を0.5時間行ってから、5%(w/w)のペプシンを加え、加水分解を0.5時間続け、続いて、5%(w/w)の複合プロテアーゼ(中性プロテアーゼ:フレーバーザイム=1:1(w/w))を加えることによって加水分解を1時間続け、この液を煮るために加熱し、20分間煮続けて上記の酵素を不活性化してから、遠心分離して不溶性不純物と脂肪を除去し、最後にこの液体を噴霧乾燥して、360gの粉末活性小分子阿膠混合物を得た。この生成物の分子量を割り出したところ、ペプチドの大半は200〜3000Daの範囲であり、全体の87%を占めた。
Example 8
1 L of glue liquid (40% (w / w)) without added auxiliary material was cooled to 40 ° C. at room temperature, and its pH was adjusted to 6.5. To this solution, 1.5% (w / w) of complex protease (papain: proline protease = 2: 1 (w / w)) was added and the hydrolysis reaction was carried out for 0.5 hour, and then 5% (w / w). by adding w) pepsin and continuing the hydrolysis for 0.5 h followed by 5% (w / w) complex protease (neutral protease: flavorzyme = 1: 1 (w / w)) Hydrolysis is continued for 1 hour, heated to boil this liquid, boiled for 20 minutes to inactivate the above enzymes, then centrifuged to remove insoluble impurities and fat, and finally the liquid is spray dried As a result, 360 g of powdered active small molecule glue mixture was obtained. When the molecular weight of this product was determined, most of the peptides ranged from 200 to 3000 Da, accounting for 87% of the total.
実施例9
補助材を加えていない1Lの阿膠液(40%(w/w))を室温で50℃まで冷まし、そのpHを6.5に調節した。この液に3%(w/w)の複合プロテアーゼ(パパイン:ペプシン:中性プロテアーゼ:フレーバーザイム:ブロメライン=6:2:2:1:1(w/w))を加え、加水分解反応を2時間行い、この液を煮るために加熱し、20分間煮続けて上記の酵素を不活性化してから、遠心分離して不溶性不純物と脂肪を除去し、最後にこの液体を噴霧乾燥して、360gの粉末活性小分子阿膠混合物を得た。この生成物の分子量を割り出したところ、ペプチドの大半は、200〜3000Daの範囲であり、全体の65%を占めた。
Example 9
1 L of glue liquid (40% (w / w)) without added auxiliary material was cooled to 50 ° C. at room temperature, and its pH was adjusted to 6.5. 3% (w / w) of complex protease (papain: pepsin: neutral protease: flavorzyme: bromelain = 6: 2: 2: 1: 1 (w / w)) was added to this solution, and the hydrolysis reaction was carried out to 2 Heat for simmering this liquid, continue simmering for 20 minutes to inactivate the above enzyme, then centrifuge to remove insoluble impurities and fat, and finally spray dry this liquid to 360 g A powdery active small molecule glue mixture was obtained. When the molecular weight of this product was determined, the majority of peptides ranged from 200 to 3000 Da, accounting for 65% of the total.
本発明の実施形態の実施例5に従って調製した粉末活性小分子阿膠混合物を下記の試験分析で用いた。 A powdered active small molecule glue mixture prepared according to Example 5 of an embodiment of the present invention was used in the following test analysis.
実施例10:活性小分子阿膠混合物中のペプチドの分布の試験
1.1:高速ゲルクロマトグラフィーを用いた試験
試験装置:
液体系:Agilent 1100、効率的なゲルカラム:TSK−G2000 SKwl(300mm×7.8mm、平均孔径500Å)
試験手順:
1mlの加水分解サンプルを量りとり、10,000gで2分間遠心分離し、上清を0.45μmの使い捨てフィルターバイアルでろ過してから、サンプルをクロマトグラフに導入した。カラム温度は27℃で、移動相は0.05モル/Lのリン酸緩衝液(pH7.2)で、その流速は0.5ml/分であり、検出波長は280nm、導入体積は20μlであった。
Example 10: Testing the distribution of peptides in active small molecule glue mixtures 1.1: Testing using high speed gel chromatography Test equipment:
Liquid system: Agilent 1100, efficient gel column: TSK-G2000 SKwl (300 mm × 7.8 mm, average pore diameter 500 mm)
Test procedure:
A 1 ml hydrolyzed sample was weighed and centrifuged at 10,000 g for 2 minutes, and the supernatant was filtered through a 0.45 μm disposable filter vial before introducing the sample into the chromatograph. The column temperature was 27 ° C., the mobile phase was 0.05 mol / L phosphate buffer (pH 7.2), the flow rate was 0.5 ml / min, the detection wavelength was 280 nm, and the introduction volume was 20 μl. It was.
1.2:遊離アミノ酸含有量の試験
試験装置:
MS:3200 Q Trap、LCシステム、Shimadzu UFLCシステム、カラム:アミノ酸分析専用のAB Sceix、ガードカラム:C18(4.0×3.0mm、5mm)、PhenomenexCo.
手順:
均一に混合した20μLの液体サンプルに5μLの沈殿剤を加え、均一に混合し、2分間、10,000gで遠心分離し、20μLの標識バッファーを5μLの上清に加え、均一になるまで混合し、2.5μLの標識試薬とともに5μLの上清を加え、均一になるまで混合し、室温で30分反応させ、反応後、2.5μLのヒドロキシルアミンを加え、均一になるまで混合し、40℃で窒素を吹き付けて乾燥し、16μLの内部標準液を加えることによって再構成し、均一になるまで混合し、16μLを量りとってサンプルバイアルに入れ、5μLをクロマトグラフに導入してアミノ酸の濃度を測定した。
1.2: Test for free amino acid content Test equipment:
MS: 3200 Q Trap, LC system, Shimadzu UFLC system, column: AB Sceix dedicated to amino acid analysis, guard column: C18 (4.0 × 3.0 mm, 5 mm), Phenomenex Co.
procedure:
Add 5 μL of precipitant to a uniformly mixed 20 μL liquid sample, mix uniformly, centrifuge at 10,000 g for 2 minutes, add 20 μL of labeling buffer to 5 μL of supernatant, and mix until uniform. Add 5 μL of supernatant with 2.5 μL of labeling reagent, mix until uniform, react at room temperature for 30 minutes, add 2.5 μL of hydroxylamine after reaction, mix until uniform, 40 ° C. Dry by blowing with nitrogen, reconstitute by adding 16 μL of internal standard solution, mix until uniform, weigh 16 μL into a sample vial, introduce 5 μL into the chromatograph and adjust the amino acid concentration. It was measured.
1.3:結果
結果は図1に示されている。図1から分かるように、サンプルは、分子量が200〜1000Daの範囲のペプチドを高い含有量(81%)で含んでおり、1000〜3000Daのペプチドの部分は全体の14%を占め、遊離アミノ酸含有量は非常に少なく、わずか4%であった。重量平均分子量は765Daであった。本発明の背景技術の部分に記載されているように、分子量が200〜1000Daのペプチドは、他のサイズのペプチド及び遊離アミノ酸と比べて吸収性と効能が高いので、他のコラーゲンペプチド生成物と比べて、本発明による生成物は、吸収速度及び機能的効能に関して優れているとみなすことができる。
1.3: Results The results are shown in FIG. As can be seen from FIG. 1, the sample contains a high content (81%) of peptides with a molecular weight in the range of 200-1000 Da, the portion of the 1000-3000 Da peptide accounts for 14% of the total and contains free amino acids. The amount was very small, only 4%. The weight average molecular weight was 765 Da. As described in the background section of the present invention, peptides having a molecular weight of 200-1000 Da are more absorbable and more effective than other sized peptides and free amino acids. In comparison, the product according to the invention can be considered excellent in terms of absorption rate and functional efficacy.
実施例11 生物学的利用能試験
材料:
通常の阿膠:通常の未処理の阿膠サンプル
生物消化した阿膠:ヒトの胃腸管での消化を模して、ペプシン及び腸内トリプシンを用いて、阿膠を酵素分解したもの
小分子阿膠:本発明で提案する方法を用いることによって得た活性小分子阿膠混合物
24匹の健常マウス(雄12匹、雌12匹、体重200〜250g)を用い、無作為にグループA、B、及びCに分けた。12時間絶食させてから投薬した。翌朝、グループAに通常の阿膠溶液、グループBに生物消化した阿膠溶液、グループCに小分子阿膠を胃内投与し(それぞれサンプル1mg/体重10g)、投与の4時間後に給餌を再開した。投与の0時間後、0.25時間後、0.5時間後、1時間後、2時間後、3時間後、4時間後、6時間後、8時間後、10時間後、12時間後、18時間後、24時間後に眼窩血液サンプルを採取した。前処理後に、アミノ酸分析を用いて血液サンプルを分析して、血中ヒドロキシルプロリン含有量を得、サンプルの生物学的利用能を標定した(ヒドロキシルプロリンは、コラーゲンの特徴的アミノ酸である)。
Example 11 Bioavailability Test Materials:
Normal glue: Normal untreated glue sample Biologically digested glue: A model of digestion of human glue in the gastrointestinal tract, using pepsin and intestinal trypsin. Small molecule glue: In the present invention Active small molecule glue mixture obtained by using the proposed method Twenty-four healthy mice (12 males, 12 females, 200-250 g body weight) were randomly divided into groups A, B, and C. The drug was administered after fasting for 12 hours. The next morning, group A was given a normal glue solution, group B was biodigested glue solution, and group C was given a small molecule glue intragastrically (each sample was 1 mg / body weight 10 g), and feeding resumed 4 hours after administration. 0 hours, 0.25 hours, 0.5 hours, 1 hour, 2 hours, 3 hours, 4 hours, 6 hours, 8 hours, 10 hours, 12 hours after administration Orbital blood samples were collected after 18 and 24 hours. After pretreatment, blood samples were analyzed using amino acid analysis to obtain blood hydroxylproline content and to standardize sample bioavailability (hydroxylproline is a characteristic amino acid of collagen).
結果は図2に示されており、図2から、本発明で提案する活性小分子阿膠混合物の生物学的利用能は、通常の阿膠の3.5倍、生物消化から得られる生成物の2.2倍であることが分かる。これらのデータにより、本発明で提案する活性小分子阿膠混合物が、小分子の特徴と高い吸収速度を有することが示された。 The results are shown in FIG. 2. From FIG. 2, the bioavailability of the active small molecule glue mixture proposed in the present invention is 3.5 times that of ordinary glue, 2 of the product obtained from biodigestion. It turns out that it is 2 times. These data indicated that the active small molecule glue mixture proposed in the present invention has small molecule characteristics and high absorption rate.
実施例12 抗酸化効果に関する試験
1.1:DPPHラジカルを除去する効果に関する調査
手順
1.5mLのサンプル溶液と1.5mLのDPPH溶液を共栓試験管に加え、遮光下で30分、振とうして反応させ、517nmにおける吸光度(AS)を測定し、同時に、0.1mモル/LのDPPH溶液1.5mLとエタノール1.5mLとの混合物の吸光度(AC)、及び、サンプル溶液1.5mLとエタノール1.5mLとの混合物の吸光度(AB)を割り出した。下記の式に従って消去率を計算した。
Example 12 Test on Antioxidant Effect 1.1: Investigation on Effect of Removing DPPH Radical Procedure Add 1.5 mL sample solution and 1.5 mL DPPH solution to a stoppered test tube and shake for 30 minutes under light shielding. The absorbance at 517 nm (A S ) was measured, and at the same time, the absorbance (A C ) of a mixture of 1.5 mL of 0.1 mmol / L DPPH solution and 1.5 mL of ethanol, and
式中、ASはサンプル溶液間の反応物質の吸光度、ACは、DPPH溶液とエタノールとの混合物の吸光度、ABは、サンプル溶液とエタノールとの混合物の吸光度である。 Wherein the absorbance of the reactant between A S sample solution, A C is the absorbance of the mixture of DPPH solution and ethanol, A B is the absorbance of the mixture of the sample solution and ethanol.
1.2:ABTSラジカルを除去する効果に関する調査
試験手順
88μLの過硫酸カリウム溶液を5mLのABTS溶液と遮光下で16時間反応させてから、吸光度が0.7±0.002になるまで、その反応物質をエタノールで希釈する。200μL(2mL)のABTS反応溶液を100μL(1mL)のサンプル溶液と96ウェルプレートで10分間反応させ、734nmにおける吸光度を測定した。下記の式に従って消去率を計算した。
1.2: Investigation on the effect of removing ABTS radicals Test procedure After reacting 88 μL of potassium persulfate solution with 5 mL of ABTS solution for 16 hours under shading, until the absorbance becomes 0.7 ± 0.002. The reaction mass is diluted with ethanol. 200 μL (2 mL) of the ABTS reaction solution was reacted with 100 μL (1 mL) of the sample solution for 10 minutes in a 96-well plate, and the absorbance at 734 nm was measured. The erasure rate was calculated according to the following formula.
式中、A0は、ABTS・+溶液の吸光度であり、Aは、サンプル溶液を加えた後のABTS・+溶液の吸光度である。 In the formula, A 0 is the absorbance of the ABTS · + solution, and A is the absorbance of the ABTS · + solution after adding the sample solution.
1.3:結果
結果は図3及び図4に示されている。図3及び4から分かるように、様々な濃度の小分子阿膠溶液の小分子はいずれも、ABTSラジカル及びDPPHラジカルを除去する効果を示し、濃度が10mg/mlの小分子阿膠溶液は、いずれのラジカルに対しても100%近い消去率を示し、本発明による生成物が一定の抗酸化効果を有することが示された。
1.3: Results The results are shown in FIG. 3 and FIG. As can be seen from FIGS. 3 and 4, the small molecules of various concentrations of small molecule glue solution all show the effect of removing ABTS radicals and DPPH radicals, and the small molecule glue solution with a concentration of 10 mg / ml It also showed an erasing rate close to 100% for radicals, indicating that the product according to the invention has a certain antioxidant effect.
Claims (11)
(1)補助材を含まない阿膠液を室温で30〜55℃まで冷まし、pHを5〜8に調節し、この液に複合プロテアーゼを加えて、加水分解反応を0.5〜2時間行うことによって、阿膠液の加水分解物を得る工程で、前記複合プロテアーゼがパパイン及びプロリンプロテアーゼを含む工程と、
(2)工程(1)で得た阿膠液の加水分解物を10〜30分間煮続けて、前記酵素を不活性化することによって、不活性化煎出物を得る工程と、
(3)前記不活性化煎出物を遠心分離して不純物を除去することによって、活性小分子阿膠混合物の液体製剤を得る工程と、
を含む方法。 A method of making the active small molecule glue mixture according to any one of claims 1, 2, or 3.
(1) Cool the glue solution not containing auxiliary materials to 30-55 ° C. at room temperature, adjust the pH to 5-8, add complex protease to this solution, and perform the hydrolysis reaction for 0.5-2 hours. By the step of obtaining a hydrolyzate of glue liquid, wherein the complex protease comprises papain and proline protease;
(2) A step of obtaining an inactivated decoction by inactivating the enzyme by continuing to boil the hydrolyzate of the glue liquid obtained in step (1) for 10 to 30 minutes;
(3) obtaining a liquid formulation of an active small molecule glue mixture by centrifuging the inactivated decoction to remove impurities;
Including methods.
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| PCT/CN2012/001566 WO2013097274A1 (en) | 2011-12-29 | 2012-11-21 | Active small-molecule donkey-hide gelatin mixture and preparation method and application thereof |
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